Occurrence and antimicrobial resistance pattern of E. coli O157:H7 isolated from foods of Bovine origin in Dessie and Kombolcha towns, Ethiopia

E. coli are frequently isolated food-borne pathogens from meat, milk, and their products. Moreover, there has been a significant rise in the antimicrobial resistance patterns of E. coli O157:H7 to commonly used antibiotics. A cross-sectional study was conducted from October 2019 to July 2021 to estimate prevalence and identify associated factors of E. coli and E. coli O157:H7 and to determine antibiotic resistance pattern of E. coli O157:H7 from foods of bovine origin in Dessie and Kombolcha towns. A total of 384 samples were collected. Systematic and simple random sampling techniques were employed for sampling carcasses and milking cows, respectively. E. coli and E. coli O157:H7 were detected according to recommended bacteriological protocols. E. coli O157:H7 strains were evaluated for in vitro antimicrobial susceptibility using agar disk diffusion method. Both descriptive and inferential statistical techniques were applied to analyze the data. Overall prevalence rates of E. coli and E. coli O157:H7 were 54.7% and 6.5%, respectively. Highest prevalence rates of E. coli (79.6%) and E. coli O157:H7 (16.7%) were obtained from carcass swabs and milk tank samples, respectively. Unlike E. coli O157:H7, a statistically significant difference in the E. coli prevalence (P<0.05) was observed among the different sample types. Multidrug resistance was observed among all isolates of E. coli O157:H7. All E. coli O157:H7 isolates (100.0%) were susceptible to Ampicillin, Sulfamethoxazole-trimethoprim, and Norfloxacin. On the contrary, all of the isolates (100%) were resistant to Penicillin G, Vancomycin, and Oxacillin. The current study indicated that different foods of bovine origin in the study area were unsafe for human consumption. Hence, good hygienic production methods should be employed to ensure the safety of foods of bovine origin.


Introduction
Analysis of food to detect food-borne pathogens is essential to ensure food safety and to reduce and/or prevent the occurrence of food-borne infections in humans [25][26][27]. Particularly, the detection of food-borne pathogenic bacteria is critical for the control and prevention of some hazardous points in food production, processing, and/or distribution [28]. However, there is insufficient information related to the occurrence of food-borne infections in developing countries though the burden is high in those countries as compared to developed countries [15]. Despite there is growing tendency of reporting E. coli O157:H7 in beef and dairy products in recent times [1], only few studies have been reported related to the epidemiology and antibiotic resistance pattern of E. coli O157:H7 in Ethiopia [13,15]. Furthermore, in most parts of Ethiopia, cow milk and beef are consumed as raw or undercooked which may prone people to pathogenic and drug-resistant food-borne bacteria. Hence, the objectives of the present study were to estimate the prevalence and identify associated factors of E. coli and E. coli O157:H7 and to determine the antibiotic resistance patterns of E. coli O157:H7 isolates from foods of bovine origin in Dessie and Kombolcha towns.

Ethics statement
This study was reviewed by the Research Ethics Review Committee of the School of Veterinary Medicine, Wollo University. The committee approved and confirmed that formal ethical approval was not required for conducting this study since it was not an experimental study and there was no risk of harm or injury to the study subjects, dairy and beef cattle, associated with the research. Prior to the investigation, the general procedures and significance of the study were explained to the study participants. Hence, the participants provided their informed verbal consent for their cattle to be included in the study. Moreover, in this study, the best practices of veterinary care were employed and all procedures were done as per the proper guidelines by professionals.

Study area
The study was conducted in Dessie and Kombolcha towns, South Wollo Zone, Eastern Amhara Region, Ethiopia (Fig 1). Dessie is the capital city of South Wollo zone which is located 401km to the northeast of Addis Ababa, the capital city of Ethiopia, and 480 km east of Bahir Dar, the capital city of Amhara Region [29]. The town is located at 11˚8'N-11˚46' North latitude and 393 8'E-41013'East longitude. Topographically, Dessie town lies within elevation range of 2,470 and 2,550 meters above sea level. It has a mean annual rainfall of 1100-1200 mm and the mean annual minimum and maximum temperatures of the town are 9˚C and 23.7˚C, respectively [30]. Administratively, Dessie town is subdivided into 18 urban and 8 rural Kebeles [31]. Kombolcha is an industrial town situated at a distance of 376 km north of Addis Ababa, the capital city of Ethiopia, 23 km south-west of Dessie, the capital city of South Wollo zone, and 505 km from Bahirdar, the capital city of Amhara Region. The town is located at 11˚6' N latitude and 39˚45'E longitude with an elevation ranges from 1, 500 to 1, 840 meters above sea level [30]. The mean annual rainfall of Kombolcha town is 1046 mm and its annual minimum and maximum temperatures are 12.9˚C and 28.1˚C, respectively. Kombolcha town has a total of 11 administrative kebeles, 6 peri-urban and 5 urban [32].
The total number of registered dairy farms in Kombolcha town at the time of sample collection was 164. In these farms, the total milking, dry and pregnant cows were 586, 266, and 386, respectively [33]. According to the document of Dessie Town Animal Production and Health Office [34], seven large-scale and well-organized dairy farms were found in Dessie town. However, 21 additional non-registered dairy farms were found in Dessie town through an assessment conducted prior to sample collection. Therefore, the total number of milking cows in the 28 dairy farms was around 196. During sample collection, only apparently healthy milking dairy cows were included. However, dry cows, heifers, and clinically ill dairy cows were excluded from the sampling.
Besides the dairy cows in the two study areas, beef cattle slaughtered at Dessie and Kombolcha municipal abbatoirs and Kombolcha ELFORA abattoir were included in the study population.

Study design
A cross-sectional study was conducted from October 2019 to July 2021 to estimate the prevalence of E. coli and E. coli O157:H7 and determine the antibiotic resistance pattern of E. coli O157:H7 from foods of bovine origin in Dessie and Kombolcha towns, Amhara, Ethiopia.

Sample size determination
The sample size (n) was determined based on a statistical formula given by Thrusfield [35].
There was no previous published report related to the proportion of E. coli and E. coli O157:H7 from foods of bovine origin in Dessie and Kombolcha towns, hence an expected prevalence (Pexp) of 50% was used for sample size calculation with 95% confidence interval and 0.05 absolute precision (d). According to the above-given formula, the total sample size computed was 384.
After the assessment of the total number of sample sources (dairy farms, milk product shops, butcher shops, and restaurants, and the number of animals slaughtered at abattoirs) in the two study sites, the sample size of each sample type was allocated proportionally. A total of 384 different samples of foods of bovine origin, including carcass swabs (n = 162) from municipal and ELFORA abattoirs, udder milk (n = 146) and milk tank (n = 6) samples from dairy farms, yoghurt (n = 36) and cottage cheese (n = 9) samples from milk product shops, and beef swabs (n = 25) from butcher shops and restaurants were collected in the two selected study settings. With respect to the study site, 203 and 181 samples were collected from Kombolcha and Dessie towns, respectively.

Sampling technique
A systematic random sampling method was employed to select carcass swab samples among cattle slaughtered at municipal and ELFORA abattoirs in study sites and every 3 rd cattle was selected. Milking cows from dairy farms in the study sites were selected using simple random sampling technique to collect udder milk samples. Moreover, tank milk, milk products (yoghurt and cottage cheese), and beef swab samples were also collected using simple random sampling technique.

Sample collection
Using sterile labeled screw cupped glass bottles, 25 ml of milk sample was collected from all quarters of the selected individual milking cows after discarding three streams of milk. Tank milk samples, around 25 ml, were also collected from dairy farms using sterile labeled screw cupped glass bottles after the milk was mixed well. From milk product shops in study sites, approximately 25 ml/g yoghurt and cottage cheese samples were collected aseptically using sterile labeled screw-capped glass bottles. At abattoirs, the carcass swab samples were collected using sterile cotton swabs from the outer and internal surface parts of the selected carcass at five separate locations (neck, thorax, abdomen, breast, and crutch). The swab samples taken from different locations of the same carcass were pooled together and dipped into labeled test tubes containing 5 ml of sterile 0.85% NaCl solution. At butcher shops and restaurants, the beef swab samples were collected from different sites of the selected individual beef and placed into labeled test tubes containing 5 ml of sterile 0.85% NaCl solution. During the time of sample collection, all necessary data related to samples such as study site, sample source, sample type, date of collection and condition of the sample sources were recorded in a pre-designed format. The samples were shipped carefully on the day of collection using an ice box containing ice packs and processed within 24 hrs in Veterinary Microbiology Laboratory, School of Veterinary Medicine, Wollo University, Dessie, Ethiopia.

Isolation and identification of E. coli and E. coli O157:H7
Detection of E. coli and E. coli O157: H7 in all collected samples was conducted according to Quinn et al. [36] with a slight modification. The bacteriological media used for isolation and identification were prepared according to the instructions of the manufacturers. After each original sample was homogenized, 1 ml of the test sample was transferred into 9 ml sterile peptone water (Micromaster, India) and incubated aerobically at 37˚C for 24 hrs. The preenriched samples were further inoculated into MacConkey broth (Blulux Laboratories Ltd., India) and incubated at 37˚C for 24 hrs for selective enrichment. The enrichments were then streaked on MacConkey Agar plates (HiMedia Laboratories Pvt. Ltd., India), and incubated at 37˚C for 24 hrs. Pink-colored colonies (Fig 2) were aseptically streaked on nutrient agar plates (HiMedia Laboratories Pvt.Ltd., India) and incubated at 37˚C for 24 hrs.
A pure colony was taken from nutrient agar plates and subjected to Gram staining as per procedures described by Merchant and Packer [37]. Gram-negative, pink-colored with rodshaped appearance and arranged in single or in pairs were suspected as E. coli. A single isolated colony was picked and streaked on Eosin Methylene Blue Agar (EMB) medium (Sisco Research Laboratories Pvt. Ltd., India) and incubated aerobically at 37˚C for 24 hrs. The presumptive E. coli colonies that showed greenish metallic sheen [38] (Fig 3) were picked up with a sterile inoculating loop and allowed to grow on nutrient agar plates (HiMedia Laboratories Pvt.Ltd., India) at 37˚C for 24 hrs for biochemical examination.
Standard biochemical tests were used for confirmatory identification of the presumptive E. coli isolates [39,40]. Slide catalase test was performed according to MacFaddin [41]; Indole test was conducted according to Cheesbrough [42]; Methyl Red and Voges Proskauer tests were  done according to Cheesbrough [42]; Citrate utilization test was performed according to Simmons [43]; Urease test for bacterial isolates was done according to Chakraborty et al. [44]; and TSI test was carried out according to Vanderzant and Splittstresser [45]. All the biochemical tests were interpreted and isolates which were indole positive, methyl red positive, Voges-Proskauer negative, citrate negative, urease negative, and producing acid with gas and without hydrogen sulfide production on TSI were confirmed to be E. coli.
E. coli O157:H7 isolates that had been confirmed biochemically were inoculated onto nutrient agar plates and incubated at 37˚C for 24 hrs. After overnight incubation, colonies were transferred and diluted into test tubes containing 5 ml of sterile 0.85% saline solution and mixed thoroughly to generate a homogeneous suspension until the turbidity of the bacterial suspension achieved the 0.5 McFarland turbidity standards. A sterile cotton swab was dipped into the adjusted bacterial suspension and the excess inoculum was removed by lightly pressing the swab against the test tube's upper inside wall.
To obtain uniform inoculums over the entire surface of the Mueller-Hinton agar plate (HiMedia Laboratories Pvt.Ltd., India), the swab containing the inoculum was spread evenly via a repeated rubbing procedure. The selected antibiotic-impregnated disks were placed at a minimum distance of 24 mm on the surface of the inoculated plate and 10 mm from the edge of the petri dish using sterile thumb forceps after the plates dried for 3 to 5 minutes and gently pressed with the point of a sterile forceps to ensure the complete contact between the disk and the agar surface. Within 15 minutes following the deposit of the disks, the plates were inverted and incubated at 37˚C for 24 hrs. After 24 hrs of incubation, the zones of growth inhibition around each of the antibiotic disks were observed. The diameters of inhibition zones were measured using a digital caliper and the findings were recorded in a pre-designed format. The inhibition zone results around individual antibiotic disks were interpreted and the isolates were classified as Sensitive (S), Intermediate (I), and Resistant (R) according to the interpretation tables of the Clinical and Laboratory Standard Institute [47][48][49][50], Arabzadeh et al. [51], Reza et al. [52], Tadesse et al. [53], and TMCC [54].

Standard organisms for quality control
To monitor the performance of the laboratory test and ensure accurate test results, the standard strains of E. coli ATCC 25922 obtained from Amhara Public Health Institute (APHI) Dessie branch, were used as control strains.

Data management and analysis
All raw data collected from the study were summarized, compiled, entered, and coded in Microsoft Excel 2007 spreadsheet and imported to STATA Version 12 software for statistical analysis. Both descriptive and inferential statistical techniques were applied to analyze and present the different data types collected from the current study. Among descriptive statistics, frequency and/or percentage were calculated. Chi-square test (χ 2 ) and binary logistic regression were computed to determine the association of different risk factors with contamination of E. coli and E. coli O157: H7 from different foods of bovine origin and the degree of association was determined using Odds ratio (OR) with 95% confidence interval (CI). Statistical significance was considered at P-value less than 0.05.
The sample type based prevalence of E. coli from carcass swab, udder milk, beef swab, tank milk, yoghurt, and cheese samples was 79.6%, 43.2%, 40.0%, 33.3%, 13.9%, and 11.1%, respectively. A statistically significant difference in the E. coli prevalence (P<0.05) was observed among the different sample types of foods of bovine origin. Among the examined sample types, the highest (16.7%) and lowest (0.0%) prevalence rates of E. coli O157:H7 were recorded from tank milk and milk products, respectively. The difference in the prevalence of E. coli O157:H7 among different sample types was not statistically significant (P>0.05) ( Table 1).
With respect to the study site, the prevalence rates of E. coli (52.5% and 56.7%) and E. coli O157:H7 (4.4% and 8.4%) were found in Dessie and Kombolcha towns, respectively. There was no statistically significant difference in the prevalence rates of the isolates between the two study sites (P>0.05) ( Table 1).
The odds of detection of E. coli were 31.27 times higher among carcass swab samples than in cheese samples and it was statistically significant (P<0.05) ( Table 2).

Prevalence of E. coli and E. coli O157:H7 among variables of different sample types
The recorded prevalence rate of E. coli O157:H7 in milk samples from cows with previous treatment history was 13.7%. The difference in the prevalence of E. coli O157:H7 among treatment history categories was statistically significant (P<0.05). The prevalence of E. coli O157: H7 from milk samples was higher in Kombolcha town (14.0%) than in Dessie town (1.9%). The difference in the prevalence of E. coli O157:H7 between the two sites was statistically significant (P<0.05) ( Table 3).
According to the result presented in Table 4, E. coli O157:H7 was not detected in milk products. The difference in the prevalence of E. coli among all hypothesized variables of milk products was not statistically significant (P>0.05).
There was no statistically significant difference in the prevalence of E. coli O157:H7 among all hypothesized variables of carcass swab samples (P>0.05). The prevalence of E. coli from carcass swab samples was higher in Kombolcha town (89.4%) than in Dessie town (72.9%) and the difference was statistically significant (P<0.05) ( Table 5).
The proportion of E. coli in beef swab samples collected from butcher shops and restaurants in Kombolcha town (66.7%) was higher than in Dessie town (15.4%) and the difference was statistically significant (P<0.05). A higher prevalence of E. coli O157:H7 (50.0%) was obtained in beef swab samples collected from butcher shops having poor hygiene and the difference was statistically significant (P<0.05) as presented in Table 6.

PLOS NEGLECTED TROPICAL DISEASES
Occurrence and antimicrobial resistance pattern of E. coli O157:H7

In vitro antimicrobial sensitivity pattern of E. coli O157:H7 isolates
The result of the in vitro antimicrobial sensitivity assay of the 25 E. coli O157:H7 isolates to the sixteen selected antimicrobial agents revealed that all strains (100.0%) were susceptible to Ampicillin, Sulfamethoxazole-trimethoprim, and Norfloxacin. On the contrary, all of the isolates (100%) were resistant to Penicillin G, Vancomycin, and Oxacillin. Moreover, high percentages of the isolates (92.0%) were also resistant to Erythromycin as presented in Table 7. Multidrug resistance to more than three drugs was observed among all isolates of E. coli O157:H7. As shown in Fig 5, 14 (56.0%) and 11 (44.0%) of the isolates showed resistance to four and five drugs, respectively.
On the other hand, the prevalence of E. coli O157:H7 found in this study was lower than the reports of Lingathurai and Vellathurai [65]  coli and E. coli O157:H7 prevalence rates between present and other previous studies might be due to differences in management and hygienic practices in dairy and beef farms, standards and furnishings of abattoir and dairy farms, dairy cow herd health status (these bacteria are commonly isolated from mastitic milk), hygienic conditions in slaughterhouses and milking premises, cleanliness of milking and slaughtering utensils, hygienic practices during milking and slaughtering, water quality and its availability, and hygienic conditions of foods of bovine origin during handling, transportation, storage, and distribution up to consumption. Moreover, the variations could also arise from differences in study methods employed by researchers including sample source, sample size, sampling techniques, sample type, and methods of detection in laboratories.
The current study showed that the prevalence of E. coli was highest in carcass swab samples (79.6%) followed by udder milk (43.2%), beef swab (40.0%), tank milk (33.3%), yoghurt (13.9%), and cheese (11.1%). Unlike E. coli O157:H7, a statistically significant difference in the E. coli prevalence (P<0.05) was observed among different sample types of foods of bovine origin. The odds of detection of E. coli were 31.27 times higher among carcass swab samples than in cheese samples and it was statistically significant (P<0.05). At abattoirs, sanitation and hygiene are the crucial factors that contribute to meat contamination [103]. Poor hygienic practices at abattoirs during bleeding, skinning, evisceration, carcass washing, and splitting might be responsible for the contamination and higher magnitude of E. coli in carcass samples. In addition, the prevalence of E. coli O157:H7 in tank milk, udder milk, carcass swab, beef swab, yoghurt, and cheese samples was 16.7%, 9.6%, 5.6%, 4.0%, 0.0%, and 0.0%, respectively. The presence of E. coli in milk is not only regarded as faecal contamination but also an indicator of poor hygiene and sanitary practices during milking and further handling [8,64,66]. The higher proportion of E. coli O157:H7 in tank milk could be from different sources including unhygienic milking practices, cows infected with mastitis, milk handlers with poor hygiene, poor quality water, and inappropriately cleaned milk filtering utensils and tanks.
The prevalence of E. coli O157:H7 from milk samples was higher in Kombolcha town (14.0%) than in Dessie town (1.9%). The statistically significant difference (P<0.05) in the prevalence of E. coli O157:H7 among the two study sites could be associated with variation in hygienic practices in the dairy environment and herd health status of dairy farms. A higher prevalence of E. coli O157:H7 was recorded in milk samples from cows with teat treatment history (13.7%) than non treated cows (2.0%) and the difference was statistically significant (P<0.05). Cows with previous mastitis history are more likely to become infected than those which had never been exposed as they might remain in a carrier state as well as the ineffectiveness of mastitis treatment medicines [104]. The most common serotypes of E. coli recovered from mastitic milk are O157, O55, O111, O124, O119, O114, O26, and O44 [105]. Thus, the relatively high magnitude of E. coli O157:H7 in milk samples from cows with treatment history might be associated with environmental bovine mastitis.
In the present study, E. coli O157:H7 was not detected in milk products. According to Rahimi et al. [106], the survival of E. coli O157:H7 in foods is dependent on the acidity of the sample; when the pH falls below 3.5, the bacteria die. Thus, the absence of E. coli O157:H7 in yogurt and cheese samples in this study might be due to the acidity of these products and the temperature used during the processing of cheese.
The prevalence of E. coli from carcass swab samples was higher in Kombolcha town (89.4%) than in Dessie town (72.9%) and the difference was statistically significant (P<0.05). The variation could be due to the difference in hygienic practices at abattoirs. The proportion of E. coli in beef swab samples collected from butcher shops and restaurants in Kombolcha town (66.7%) was higher than in Dessie town (15.4%) and the difference was statistically significant (P<0.05). The variation could be due to the difference in hygienic practices during the slaughtering process at abattoirs and sanitation at butcher shops and restaurants. Moreover, a higher prevalence of E. coli O157:H7 (50.0%) was obtained in beef swab samples collected from butcher shops having poor hygiene and the difference was statistically significant (P<0.05). The higher occurrence of E. coli O157:H7 in beef swab samples collected from butcher shops having poor hygiene was not surprising since beef contamination is usually associated with poor hygiene.
The occurrence of antimicrobial resistance among foodborne pathogens is increasing [107]. The E. coli O157:H7 strains are heterogeneous with respect to antibiotic resistance [108]. The development of antimicrobial resistance in E. coli O157:H7 strains isolated from animals and humans [90] and the emergence of multidrug-resistant E. coli O157:H7 strains become a universal public health concern [109]. In the present study, multidrug resistance to more than three drugs was observed among all E. coli O157:H7 isolates. In brief, 56.0% and 44.0% of the isolates showed resistance to four and five drugs, respectively.
All isolates of E. coli O157:H7 (100%) were resistant to Penicillin G, Vancomycin, and Oxacillin. Moreover, high percentages of the isolates (92.0%) were also resistant to Erythromycin. The total resistance to Penicillin G was similar to the reports of Igbinosa and Chiadika [110] and Reuben et al. [111] who reported 100.0% resistance to Penicillin G in Benin City (Nigeria) and Nasarawa State (Nigeria), respectively. However, Msolo et al. [112] reported 85.0% resistance to Penicillin G in South Africa. The resistance of all isolates to Vancomycin was comparable to the report of Bedasa et al. [19] who reported 90.0% resistance to Vancomycin in Bishoftu town. The high frequency of resistance to Erythromycin was in agreement with the previous reports of Reuben and Owuna [90] in Nasarawa State, Nigeria, and Igbinosa and Chiadika [110] in Benin City (Nigeria) who reported 94.7% and 89.5% resistance to Erythromycin, respectively. The total resistance of the isolates to Oxacillin was higher than the report of Reuben and Owuna [90] who reported 84.2% resistance to Oxacillin.
On the contrary, all E. coli O157:H7 strains (100.0%) were susceptible to Ampicillin, Sulfamethoxazole-trimethoprim, and Norfloxacin. The total susceptibility to Sulfamethoxazole-trimethoprim was similar to previous findings of Tadese et al. [76], Bekele et al. [10], Beyi et al. [89], and Geresu and Regassa [96] who reported 100.0% sensitivity to Sulfamethoxazole-trimethoprim in Ambo town, Addis Ababa, central Ethiopia, and selected study settings of Arsi Zone, respectively. The total susceptibility to Norfloxacin was similar to the previous finding of Tadese et al. [76] (100.0%) in Ambo town. The 100.0% susceptibility to Ampicillin was similar to the previous report of Osaili et al. [113] who reported 100.0% sensitivity to Ampicillin in Amman City, Jordan.
Higher percentages of the isolates were also sensitive to Doxycycline (92.0%), Tetracycline (96.0%), Ceftriaxone (96.0%), Gentamicin (88.0), Nalidixic acid (88.0%), Amikacin (72.0%), and Ciprofloxacin (72.0%). The sensitivity of isolates to Gentamicin was comparable with the report of Bedasa et al. [19] who reported 82.5% sensitivity to Gentamicin in Bishoftu town. The susceptibility to Amikacin was consistent with Msolo et al. [112] who reported 70.0% sensitivity to Amikacin in South Africa. The sensitivity to Ciprofloxacin was consistent with the reports of Bekele et al. [10] in Addis Ababa and Reuben and Owuna [90] in Nasarawa State, Nigeria who reported 76.5% and 78.9% sensitivity to Ciprofloxacin, respectively. The high sensitivity to Ceftriaxone was consistent with the reports of Bedasa et al. [19], Atnafie et al. [13], and Haile et al. [114] who reported 100% sensitive isolates to Ceftriaxone in Bishoftu, Hawassa, and Jimma towns, respectively. The 96.0% sensitivity to Tetracycline was consistent with Haile et al. [114] in Jimma, Bekele et al. [10] in Addis Ababa, Osaili et al. [113] in Amman City (Jordan), and Bedasa et al. [19] in Bishoftu town who reported 100%, 100.0%, 100.0% and 97.5% sensitivity to Tetracycline. However, Welde et al. [87] reported 77.8% resistance to Tetracycline in and around Modjo town. According to Mokgophi et al. [115] and Qamar et al. [116], the extensive, indiscriminate and injudicious use of antibiotics in both veterinary medicine and public health leads to genetic modification in most bacterial strains for evolving resistance and an increase in the prevalence of resistance among pathogens.

Conclusion and recommendations
The high magnitude of E. coli contamination and finding of multidrug-resistant E. coli O157: H7 in the current study indicated that different foods of bovine origin in the study area were unsafe for human consumption. The multidrug resistance pattern of all E. coli O157:H7 isolates might be due to the injudicious and extensive use of antibiotics in both veterinary and human medicines. In addition, slaughtering of cattle on the floor at municipal abattoirs, unsanitary milk production, and handling, and the community's consumption habit of raw animal products could expose humans in study sites to multidrug-resistant E. coli O157:H7. However, the current study didn't address the serotyping and molecular characterization of E. coli O157:H7 and its antimicrobial resistance genes. Hence, good hygienic production methods should be employed to ensure the safety of different foods of bovine origin. Microbiological guidelines mainly the HACCP system and standardized slaughtering operations should be followed to improve meat safety. The emergence and spread of antibiotic-resistant pathogens should be assessed regularly and rational use of antibiotics should be practiced. Moreover, further studies on serotyping and molecular characterization of E. coli O157:H7 should be done at the study sites.